Development of a liposome-based immunochromatographic strip assay for the detection of Salmonella

Development of a liposome-based immunochromatographic strip assay for the detection of Salmonella

Salmonella species are ubiquitous human pathogens which pose a dangerous threat to the elderly and children worldwide. In this study, to develop a more efficient assay procedure for the rapid detection of Salmonella Typhimurium, an immunochromatographic strip assay was developed using immunoliposome...

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Veröffentlicht in:Analytical and bioanalytical chemistry 2011-11, Vol.401 (8), p.2581-2590
Hauptverfasser: Shukla, Shruti, Leem, Hyerim, Kim, Myunghee
Format: Artikel
Sprache:eng
Schlagworte:
Analytical Chemistry
Antigens
Assaying
Biochemistry
Characterization and Evaluation of Materials
Chemistry
Chemistry and Materials Science
Chromatographic methods and physical methods associated with chromatography
Exact sciences and technology
Fluorescence
Food Science
Goats
Humans
Immunoassay - economics
Immunoassay - methods
Immunochromatography - economics
Immunochromatography - methods
Immunoglobulin G
Laboratory Medicine
Liposomes
Liposomes - immunology
Mathematical analysis
Miscellaneous
Monitoring/Environmental Analysis
Original Paper
Other chromatographic methods
Phospholipids
Salmonella
Salmonella food poisoning
Salmonella Infections - diagnosis
Salmonella Infections - immunology
Salmonella typhimurium
Salmonella typhimurium - immunology
Salmonella typhimurium - isolation & purification
Sensitivity and Specificity
Spectrometric and optical methods
Strip
Time Factors
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Zusammenfassung:Salmonella species are ubiquitous human pathogens which pose a dangerous threat to the elderly and children worldwide. In this study, to develop a more efficient assay procedure for the rapid detection of Salmonella Typhimurium, an immunochromatographic strip assay was developed using immunoliposome (anti- Salmonella IgG-tagged) encapsulated with sulforhodamine B (SRB). The detection sensitivity of the developed immunochromatographic assay was compared with a commercial immunochromatographic test strip using colloidal gold nanoparticles. The liposomes were prepared through a reverse-phase evaporation method by using a lipid and phospholipid mixture and SRB, a fluorescence dye, which was encapsulated in the phospholipid bilayer. Furthermore, the outer surface of the SRB-encapsulated liposome was conjugated with antibody (affinity-purified polyclonal goat anti- Salmonella IgG) to form an immunoliposome (size, 223 nm), used as the analytical reagent in the developed immunoassay. For this strip assay, a plastic-backed nitrocellulose strip was immobilized with two antibody zones. The lower zone of the strip referred to Salmonella antigen capture zone (test line), while the other zone served as a positive control (control line). The lower zone was coated with affinity-purified polyclonal goat anti- Salmonella IgG, while the upper zone was coated with rabbit anti-goat IgG. During capillary migration of the wicking solution (diluted liposome and Salmonella culture, each 50 μl), Salmonella was captured with surface-bound immunoliposomes at the antigen capture zone, while the unbound liposomes migrated upward and bound to another zone. The color density of the antigen capture zone was directly proportional to the amount of S. Typhimurium in the test sample. As a result, the detection limit of the immunochromatographic strip assay developed in this study against S . Typhimurium was found to be 10 2  CFU/ml, which was significantly higher than the detection limit (10 7  CFU/ml) of the commercial immunochromatographic test strip assay. Figa The concept of immunochromatographic strip assay
ISSN:1618-2642
1618-2650
DOI:10.1007/s00216-011-5327-2